Dynamic changes in peripheral lymphocytes and antibody response following a third dose of SARS-CoV-2 mRNA-BNT162b2 vaccine in cancer patients

The aim of this study was to evaluate the association of circulating lymphocytes profiling with antibody response in cancer patients receiving the third dose of COVID-19 mRNA-BNT162b2 vaccine. Immunophenotyping of peripheral blood was used to determine absolute counts of lymphocyte subsets, alongside detection of IgG antibodies against receptor-binding-domain (RBD) of the SARS-CoV-2 Spike protein (S1) before booster dosing (timepoint-1) and four weeks afterward (timepoint-2). An IgG titer ≥ 50 AU/mL defined a positive seroconversion response. An IgG titer ≥ 4446 AU/mL was assumed as a correlate of 50% vaccine efficacy against symptomatic infections. A total of 258 patients on active treatment within the previous six months were enrolled between September 23 and October 7, 2021. The third dose resulted in an exponential increase in median anti-RBD-S1 IgG titer (P < 0.001), seroconversion rates (P < 0.001), and 50% vaccine efficacy rates (P < 0.001). According to ROC curve analysis, T helper and B cells were significantly associated with seroconversion responses at timepoint-1, whereas only B cells were relevant to 50% vaccine efficacy rates at timepoint-2. A positive linear correlation was shown between anti-RBD-S1 IgG titers and these lymphocyte subset counts. Multivariate analysis ruled out a potential role of T helper cells but confirmed a significant interaction between higher B cell levels and improved antibody response. These findings suggest that peripheral counts of B cells correlate with humoral response to the third dose of mRNA-BNT162b2 vaccine in actively treated cancer patients and could provide insights into a more comprehensive assessment of vaccination efficacy.

www.nature.com/scientificreports/ patients, including those on active cancer treatments. The paucity of data on its immunogenicity is inconsistent with the rapid deployment of this preventive measure 10 . The availability of biomarkers predicting the clinical efficacy of vaccination is also a controversial issue 11 . Most of the research focused on determining an optimal antibody titer threshold, as higher levels have been thought to be associated with neutralization capacity and lower risk of symptomatic infection 12,13 . Nevertheless, a reliable correlate of humoral response for this purpose remains ill-defined 14 . In this context, the vaccine-induced cell-mediated immune response has been considered essential for humoral immunity and clinical protection even in high-risk conditions 15,16 . However, its role has been less thoroughly characterized, with few studies investigating SARS-CoV-2-specific T and B cell responses after fulldose vaccination [17][18][19][20] . More recent data suggest that absolute counts of circulating lymphocyte subsets were associated with vaccine response in a highly vulnerable population receiving CD20 B-cell depletion treatments 21,22 , but their role has never been investigated in patients with solid tumors on active systemic therapies.
To address these issues, the Vax-On-III-Profile study prospectively assessed the potential association of circulating lymphocyte subset counts with antibody response and vaccine efficacy correlates in actively treated cancer patients receiving the third dose of tozinameran.

Methods
Design and participants. The Vax-On-III-Profile was a prospective, single-center, observational cohort study. The referring Ethics Committee approved this experimental project (Comitato Etico Lazio 1, Rome, Italy; protocol Number: 1407/CE Lazio1). The study protocol adheres to the reporting guidelines for Strengthening the Reporting of Observational Studies in Epidemiology (STROBE) and received formal registration (clinical trial identifier: EudraCT Number 2021-002,611-54). The main eligibility requirements included age ≥ 18 years, histological diagnosis of solid tumor, active oncologic treatment underway or completed within the previous six months, and fulfillment of the two-dose series of tozinameran at least 22 weeks before enrollment. The exclusion criteria comprised life expectancy < 12 weeks, active and concomitant hematological malignancy, documented COVID-19 infection at any time, and pregnancy. Eligible patients received 30 μg of tozinameran intramuscularly at least 24 h apart from their expected anticancer treatment (timepoint-1). Blood samples for serological and immunological testing were collected at timepoint-1 and four weeks afterward (timepoint-2). Adherence to vaccination was voluntary and carried out after the acquisition of institutional informed consent. All participants gave specific written informed consent for the study proposal and procedures, but their participation was not a prerequisite for receiving the booster dose. The methods used in this study comply with the tenets of the 1964 Declaration of Helsinki and its subsequent amendments, and were performed in accordance with the relevant guidelines and regulations.
The first co-primary endpoint was the correlation of dynamic changes in circulating lymphocyte counts with IgG antibody titers against the receptor-binding domain (RBD) of the SARS-CoV-2 Spike protein (S1) and seroconversion responses. The second co-primary endpoint was to determine whether lymphocyte subpopulation dynamics could show an independent interaction with antibody and seroconversion responses. As of November 10, 2021, the data would be considered conclusive.
Serological test. Whole blood samples were collected (3 mL/subject in BD Vacutainer Plus Plastic Serum Tubes) and separated by immediate centrifugation. Serum specimens were analyzed at each sampling. The SARS-CoV-2 IgG II Quant assay on the ARCHITECT i2000sr automated platform (Abbott Laboratories, Diagnostics Division, Sligo, Ireland) was used to detect anti-RBD-S1 IgG antibodies according to the manufacturer's instructions 23 . The results were reported as arbitrary units (AU)/mL, with a cut-point ≥ 50 AU/mL indicating a positive seroconversion response. In addition, an anti-RBD-S1 antibody titer ≥ 4446 AU/mL was assumed as a reliable threshold associated with 50% vaccine efficacy against a symptomatic COVID-19 infection. Since the study by Feng et al. 12 from which we derived this correlate employed a different immunoassay, we did not perform any direct assessment of the clinical efficacy of the third dose of tozinameran as related to this parameter. On the basis of adequate correlation with the serological test in our study 24 , we instead chose this threshold because it was considered an immune response more suitable than the seroconversion with respect to antibody titer levels induced by booster dosing.
Immunophenotyping. Whole blood draws for flow cytometry analysis (3 mL/subject in BD Vacutainer spray-coated K2EDTA Tubes) were collected at the same time as sampling for serological testing. The panel for staining included the following monoclonal antibodies: CD3 FITC, CD4 PE-Cy7, CD8 APC-Cy7, CD19 APC, CD45 PerCP-Cy5.5, and CD16 PE + CD56 PE; BD Biosciences, San Jose, CA). As we have previously described 25 , the BD Multitest 6-color TBNK reagent was used to determine absolute counts of B and NK cells, as well as CD4 and CD8 subpopulations of T cells. The data were collected using the BD FACSCanto II system and BD FACSCanto clinical software (BD Biosciences, San Jose, CA) as directed by the manufacturer 26 .The results were reported as absolute cell counts/µL for each lymphocyte subset. An example of the gating strategy is shown in Supplementary Fig. 1 www.nature.com/scientificreports/ oid therapy, type and timing of active treatments. At both time points, receiver operating characteristic (ROC) curves were calculated to determine the sensitivity and specificity of peripheral blood lymphocyte subsets in relation to positive seroconversion responses. Variables with a statistically significant association to the intended outcome were considered relevant for subsequent evaluations. The Youden index was applied to determine the optimal cut-point. The Spearman method was used to assess the correlation between the log values anti-RBD-S1 IgG titers and significant lymphocyte subset counts. A secondary multivariate analysis was performed by fitting the same model to anti-RBD-S1 IgG log titers and seroconversion responses or 50% vaccine efficacy rates as a function of circulating lymphocyte levels in addition to independent covariates described above. All tests performed were two-sided and a P value < 0.05 was considered significant. SPSS (IBM SPSS Statistics for Windows, version 23.0, Armonk, NY) and Prism (GraphPad, version 9) software were used for statistical evaluations and figure rendering, respectively.

Results
Patient characteristics. This study enrolled 258 consecutive patients who met the inclusion criteria and received a third dose of tozinameran between September 23 and October 7, 2021. The entire population consisted of 202 (78.3%) patients who had previously participated in the Vax-On study 27 and 56 (21.7%) cases who were recruited at a later time point. The patients' flow diagram depicts the reasons why a portion of the original study population did not receive the third dose of tozinameran ( Supplementary Fig. 2 Dynamic changes in peripheral lymphocyte counts. Peripheral blood immunophenotyping was completed in 256 (99.2%) and 251 (97.2%) patients at timepoint-1 and -2, respectively (Supplementary Fig. 2). We observed a considerable variability in the values of each subset of lymphocytes among patients, which even increased after the booster dose. Compared with baseline, the third dose of tozinameran did increase the median values of all lymphocyte subsets. This difference was statistically significant only for T cytotoxic (P = 0.001) and NK cells (P < 0.001, Fig. 1). In view of their potential effect on lymphocyte composition, we performed the same comparative evaluation according to the different types of active treatments and corticosteroid therapy. The incremental variation induced by the booster dose was confirmed in all subgroups. Of note, an increase in both T cytotoxic and NK cells was significant only in patients receiving cytotoxic chemotherapy or its combination with biological agents ( Supplementary Fig. 3). The same result was also found in patients who were not being treated with corticosteroids at immunosuppressive dosage levels before the third dose of tozinameran (Supplementary Fig. 4). We also performed a preliminary multivariate analysis to verify the effects of independent clinical variables on lymphocyte subset counts at timepoint-1. Immunosuppressive corticosteroid therapy before the third dose correlated with lower counts in T helper (P < 0.001) and B cells (P = 0.017), whereas no significant interaction was found with types or timing of active treatments (Supplementary Table 1).

ROC curves and correlation analysis. An initial ROC curve was calculated to establish the relation-
ship between lymphocyte subset counts before booster dosing and seroconversion responses at timepoint-1. T helper and B cell subpopulations showed a significant association and were found to be valuable in predicting the likelihood of a positive outcome ( Fig. 2A). With a cut-off value of 441/µL for T helper and 58/µL for B cells, the sensitivity and specificity were 0.74 and 0.54, and 0.76 and 0.62, respectively. Evaluating anti-RBD-S1 log IgG titers as a function of these lymphocyte log counts demonstrated a significant positive linear correlation for either T helper [ρ = 0.15 (95% CI 0.02-0.27), P = 0.012; Fig. 3A] and B cell subpopulation [ρ = 0.19 (95% CI 0.06-0.33), P = 0.001; Fig. 3B]. Given that almost all patients achieved a seroconversion response at timepoint-2, a subsequent ROC curve analysis was computed to determine the relationship between lymphocyte subset counts after booster and 50% vaccine efficacy at the same time point. Only the subset of B cells revealed a significant association and was therefore deemed relevant for subsequent evaluations (Fig. 2B). The cut-point value of 77/ µL defined sensitivity and specificity levels of 0.68 and 0.57, respectively. In contrast to the findings for T cell log counts [ρ = 0.09 (95% CI -0.04 -0.21), P = 0.14; Fig. 3C], a significant positive linear correlation was confirmed between anti-RBD-S1 log IgG titers and B cell log counts at timepoint-2 [ρ = 0.22 (95% CI 0.09-0.34), P < 0.001; Fig. 3D]. We also performed the same correlation analysis in subgroups of patients featuring the same active treatment at both time points (Supplementary Figs. 5 to 10). It is worth noting that the B lymphocyte subpopulation showed higher coefficients at timepoint-1 and/or 2, confirming previous results.
Analysis of antibody response. ROC   www.nature.com/scientificreports/ of antibody titers, seroconversion rates, and 50% vaccine efficacy rates at timepoint-2. After booster dosing, the high-level B cell subset also had significantly increased antibody titers and 50% vaccine efficacy rates (Table 2 and Fig. 4). All breakthrough infections occurred in the subgroup of patients with low-level B cell counts at both time points (P < 0.001). The subgroups defined by T helper and B cell levels at timepoint-1, as well as B cell levels at timepoint-2, were included in the multivariate testing as independent covariates. Different T helper cell levels at timepoint-1 were not found to be associated with any of the immune parameters. High-level B cell counts before the third dose of vaccine were confirmed to be significantly correlated with both an improved humoral response before the booster dose (P = 0.047) and increased 50% vaccine efficacy rates at timepoint-2 (P = 0.007). High-level B cell counts after the booster dose resulted in a significant interaction with either increased antibody titers (P = 0.01) and 50% vaccine efficacy rates at timepoint-2 (P = 0.003). While types and timing of active treatments did not show a reliable influence, immunosuppressive corticosteroid therapy and ECOG PS2 had detrimental effects on antibody responses at both time points (Table 3).

Discussion
The Vax-On-III-Profile is a longitudinal interventional study investigating the predictive value of dynamic changes in peripheral lymphocyte subsets on humoral response to the third dose of tozinameran. To our knowledge, this is the first study evaluating these biomarkers and vaccine efficacy in patients with solid malignancies receiving active treatments. The third dose of tozinameran induced a 34-fold increase in the median anti-RBD-S1 IgG titer. This change led to an outright improvement in seroconversion rates by 10%, with only a few patients (1.2%) remaining seronegative 28 days after the booster dosing. An antibody response of this magnitude is overlaid by that described in similar studies that employed the same serologic testing methodology 28,29 . This enhanced humoral immunity also appears to be consistent with the results of two studies showing that mRNA-vaccine booster dosing induces a strengthened neutralizing antibody response against VOCs in cancer patients 30,31 . Our additional analysis aimed to overcome the misleading value of the seroconversion response, which was developed as a diagnostic tool for prior SARS-Cov-2 exposure but has never been correlated to a protective clinical effect 32 . The minimum antibody titer required to protect against symptomatic SARS-Cov-2 infection is unknown but presumably higher than the seroconversion cut-off 12 . Assuming that a 50% vaccine efficacy-related antibody titer indicates an intermediate level of clinical protection, the booster dose would have reduced the risk of symptomatic infection in more than 76% of patients.
The positive correlation of baseline B cell counts with anti-RBD-S1 IgG titers at both time points suggests a direct relationship between these immune parameters. The significant association between incremental variations  [17][18][19][20]33 and high-resolution flow cytometry assays incorporating multiple cytokines and activation markers for RBD-S1-specific memory B cell profiling 17 . Although these assays are ideal because of their high sensitivity and specificity, the suboptimal level of procedure standardization and methodological complexities still prevent their widespread use. Immunophenotyping of peripheral blood in this study provides a nonspecific description of lymphocyte response to tozinameran booster vaccination. This approach has inherent strengths and weaknesses. The main advantage of this methodology is the high level of procedure standardization and reproducibility of the results, as it is commonly used for the diagnosis and monitoring of hematologic malignancies and is available in most facilities 34 . However, peripheral lymphocyte counts may be influenced by vaccine-independent variables, the most relevant of which are the effects of different types and timing of cancer treatments 35,36 . Preliminary multivariate analysis ruled out a selection imbalance due to direct interaction with the above factors but showed a significant effect of immunosuppressive corticosteroid dosing on T helper and B cell counts. The unavailability of comparable studies in patients with solid malignancies makes it challenging to determine the clinical significance of our findings. Even so, several studies have found a direct correlation between vaccine-induced absolute T helper and B cell counts and anti-spike IgG antibody titers in patients on CD20 B-cell-depleting treatments 21,22,37 . There was also a high concordance between SARS-CoV-2-specific T and B cell reaction testing and circulating lymphocyte immunophenotyping results. Given the differences among patients with hematologic and solid malignancies, the described experimental evidence is consistent with our findings, confirming the validity of this methodological approach to adaptive immunity associated with tozinameran vaccination. In addition to the above methodological issues, this study recognizes further shortcomings. The experimental design could not include a control group of age-and sex-matched healthy volunteers since booster vaccination had not yet been licensed for these categories at accrual time. The health contingency accounted for "all-comers" enrollment but did not allow for adequate stratification of participants. This flaw increased the likelihood of selection bias and false-positive results from multivariable statistical comparisons, the significance of which should therefore be considered as hypothesis-generating. The measurement of anti-RBD-S1 IgG titers and assumption of 50% vaccine efficacy relied on the wild-type SARS-CoV-2 strain, which could not account for the high evasive capacity of subsequent Omicron VOC spread 38,39 . In this regard, the use of an assay for neutralizing activity of vaccine-induced antibody levels would have been optimal, but procedural constraints prevented us from implementing this method of investigation 40 . Finally, although we found a significant difference in the clinical Table 2. Univariate analysis of antibody response. Statistically significant P values are highlighted in bold. Differences between groups were assessed using the Mann-Whitney U test (continuous variable) or the Pearson's χ 2 test (categorical variables), as appropriate. A two-sided P value of < 0.05 was considered statistically significant. IgG, immunoglobulin G; AU, arbitrary unit; CI, confidence intervals. a Seroconversion response at cut-off ≥ 50 AU/mL; b 50% vaccine efficacy at cut-off ≥ 4446 AU/mL; Timepoint-1 denotes antibody response assessment six months after starting vaccination; Timepoint-2 denotes antibody response assessment four weeks after the third dose of tozinameran. www.nature.com/scientificreports/ outcome of vaccination, the rate of breakthrough infections is still too low (< 4%). This finding may support vaccine efficacy itself or, more likely, reflects the effects of non-pharmaceutical interventions.

Conclusion
This cohort study confirms the enhanced immunogenicity and, presumably, clinical efficacy of the third dose of tozinameran in an extensive unselected population that may adequately represent cancer patients treated in the real world. Our data suggest that dynamic changes in circulating B lymphocyte counts, as assessed by widely available immunophenotyping of peripheral blood, correlate with the reliability of antibody response. Although Intervals. Differences between groups were assessed using the Mann-Whitney U test (continuous variable) or the Pearson's χ 2 test (categorical variables), as appropriate. A two-sided P value of < 0.05 was considered statistically significant. RBD-S1, receptor-binding domain (RBD) of the SARS-CoV-2 Spike protein (S1); AU, Arbitrary Unit; log, logarithmic values. Timepoint-1 denotes assessment before the third dose of tozinameran; Timepoint-2 denotes assessment four weeks after the third dose of tozinameran; an antibody titer ≥ 50 AU/ mL indicates a positive seroconversion response; antibody titer ≥ 4446 AU/ml was associated with 50% vaccine efficacy against a symptomatic COVID-19 infection. www.nature.com/scientificreports/ unrelated to antibody response, the significant increase in T cytotoxic and NK cells induced by the booster dose deserves further investigation of their potential effects on anticancer treatment outcomes. The limitations described warrant confirmation by independent prospective cohorts. Upon validation and longer follow-up of clinical events, our results could provide insights into a more comprehensive assessment of the efficacy of SARS-CoV-2 vaccination with respect to further active immunization strategies.